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Proteomics Extraction of Plant Protein Methodology for the Extraction of Plant Protein Extraction of total protein from the sample requires an optimized protocol. Many protocols have been developed to increase the amount of protein in the extract form different samples. The method explained here focuses mainly on extracting protein from plant tissue. Learning Objectives: After interacting with this learning object, the learner will be able to: Describe extraction of plant protein using lysis buffer. Solubilise the plant protein using rehydration buffer. Interpret the results of the experiment. Troubleshoot at various steps in the experiment. Note: The current IDD exists in two modes- interactive and automatic. Students taking lab course should select interactive (set as default), while the automatic mode may be selected for general users.

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Proteomics

Extraction of Plant Protein

Methodology for the Extraction of Plant Protein

Extraction of total protein from the sample requires an optimizedprotocol. Many protocols have been developed to increase theamount of protein in the extract form different samples. Themethod explained here focuses mainly on extracting protein fromplant tissue.

Learning Objectives:

After interacting with this learning object, the learner will be able to:

• Describe extraction of plant protein using lysis buffer.

• Solubilise the plant protein using rehydration buffer.

• Interpret the results of the experiment.

• Troubleshoot at various steps in the experiment.

Note: The current IDD exists in two modes- interactive and automatic.Students taking lab course should select interactive (set as default),while the automatic mode may be selected for general users.

Extraction of Plant Protein

Clean the surface of the balance with a tissue.

Place a butter paper and tare the weight of the paper.

Reagents Preparation

Extraction of Plant Protein

Weigh 1g of Trichloro acetic acid, 0.007 g ofDithiotreitol and add 10 ml of Acetone to prepare lysisbuffer.

Vortex the tube well to completely dissolve thecontents and store it at 4 degree C for use later.

Reagents Preparation

Extraction of Plant Protein

Prepare wash buffer by weighing 0.07 g ofDithiotreitol and dissolve it in 10ml of acetone.

Vortex the contents of the tube to mix thoroughly.Store the wash buffer so formed at 4 degree C forfurther use.

Reagents Preparation

Extraction of Plant Protein

Weigh 0.02 g of CHAPS, 0.6 g of Urea and dissolve it inwater.

Vortex the contents to mix thoroughly.

Reagents Preparation

Extraction of Plant Protein

Add 0.05% bromophenol blue to the rehydrationbuffer. It helps in tracking the sample duringelectrophoretic run.

Vortex the contents again for thorough mixing.

Reagents Preparation

Extraction of Plant Protein

Place the isolated leaves in a petriplate.

Wash the leaves with distilled water to remove all theparticulate matter on the surface. Repeat it as manytimes as required without being too harsh till theleaves are completely clean.

Once clean, dry the leaves on a tissue paper without applying excess pressure.

Cleaning and weighing of Leaves

Extraction of Plant Protein

After the leaves are totally dry, weigh the requiredamount on a balance.

Cleaning and weighing of Leaves

Extraction of Plant Protein

Take a mortar and pestle. Wipe the inside of themortar and the surface of the pestle with a tissuepaper and place it on ice.

Pour liquid nitrogen into the mortar. This is done topre-chill the mortar for further treatment.

Liquid Nitrogen Treatment

Extraction of Plant Protein

Transfer the leaves into the pre-chilled mortar.

Liquid Nitrogen Treatment

Extraction of Plant Protein

Add around 10 ml of liquid nitrogen to the mortarcontaining leaves, all at one go. A crackling sound isheard on addition of liquid nitrogen to the leaves.

Liquid Nitrogen Treatment

Extraction of Plant Protein

Grind the leaves till a fine powder is seen. The finerthe powder the better it is for protein extraction.

Grinding the Leaves

Extraction of Plant Protein

To the powdered leaves, add lysis buffer and grind thoroughly.

Lysis buffer helps in complete lysis of the cells andhence bears a lot of significance in the protocol.

Lysis Buffer Treatment

Extraction of Plant Protein

To the thick paste in the mortar, add lysis buffer andgrind thoroughly.

Transfer the lysate from the mortar to fresh eppendorftubes. Scrape out the mortar to remove any tissue leftout.

Add some more lysis buffer to the tube containing thelysate, to ensure proper lysis of cells. Vortex the tubethoroughly to mix the contents uniformly.

Lysis Buffer Treatment

Extraction of Plant Protein

After vortexing the contents of the tube, incubate thetube at -20°C for one hour.

The proteins at the end of this incubation, getprecipitated in the buffered solution.

Protein Precipitation at -20°C

Extraction of Plant Protein

Take the tube out of -20 degree C freezer. Now, place the tube in the centrifuge.

Set the parameters like speed, temperature andduration to 14000rpm, 4 degrees C and 30minutes,respectively.

Centrifugation and Acetone Wash

Extraction of Plant Protein

Take the tube out of the centrifuge. The tube can beseen to have a clearly demarcated pellet andsupernatant.

Discard the supernatant carefully without disturbingthe pellet.

Centrifugation and Acetone Wash

Extraction of Plant Protein

To the pellet, add 1ml of wash buffer. Wash bufferhelps in removing the color of the pellet.

Centrifugation and Acetone Wash

Extraction of Plant Protein

Vortex the tube to thoroughly let the pellet dissolveinto the buffer. Incubate the tube in the -20 degreefreezer for 30 minutes.

Centrifugation and Acetone Wash

Extraction of Plant Protein

Remove the tube from the freezer carefully.Centrifuge the tube at 14000rpm, 4 degrees C for 15minutes.

Discard the supernatant carefully without disturbingthe pellet. Air dry the pellet to remove even traces ofacetone.

Centrifugation and Acetone Wash

Extraction of Plant Protein

Add 400 μL of rehydration buffer to the air-driedpellet.

Vortex the tube till the pellet dissolves in the rehydration buffer.

Rehydration buffer consists of CHAPS which solubilisesthe proteins and Urea which denatures the proteins.

Rehydration Buffer Treatment

Extraction of Plant Protein

Incubate the tube overnight at 4 degree C forcomplete solubilisation of proteins in the rehydrationbuffer.

Rehydration Buffer Treatment

Extraction of Plant Protein

The sample if not required immediately can be storedat -20°C for later use.

For more information and continuity please go throughthe following IDDs.

Sample Storage